US20090263903A1 - Method for determining prothrombin time - Google Patents

Method for determining prothrombin time Download PDF

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US20090263903A1
US20090263903A1 US11/909,208 US90920806A US2009263903A1 US 20090263903 A1 US20090263903 A1 US 20090263903A1 US 90920806 A US90920806 A US 90920806A US 2009263903 A1 US2009263903 A1 US 2009263903A1
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Juha Horsti
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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/56Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving blood clotting factors, e.g. involving thrombin, thromboplastin, fibrinogen
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/86Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving blood coagulating time or factors, or their receptors
    • YGENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
    • Y10TECHNICAL SUBJECTS COVERED BY FORMER USPC
    • Y10TTECHNICAL SUBJECTS COVERED BY FORMER US CLASSIFICATION
    • Y10T436/00Chemistry: analytical and immunological testing
    • Y10T436/11Automated chemical analysis

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  • the present invention relates to tests based on INR units for monitoring oral anticoagulation therapy and hepatocellular carcinoma (HCC).
  • HCC hepatocellular carcinoma
  • the invention provides a method for determining prothrombin time of a plasma or whole blood sample taking account the effect which protein induced by vitamin K absence or antagonists (Pivka) has on INR.
  • the object of the invention is to harmonise prothrombin time methods for international normalized ratio (INR) results and also measure Pivka effect as INR units (i.e. INR Pivka ).
  • the prothrombin time (PT) test was introduced to control oral anticoagulant therapy (OAT), which is used to treat patients with thrombotic disorders such as thrombophilia.
  • OAT oral anticoagulant therapy
  • This therapy is based on vitamin K antagonists such as warfarin (or coumarin) inhibiting the synthesis of coagulation factors (F II, F VII, F IX and F X) in the liver.
  • warfarin or coumarin
  • the most commonly used PT tests are based on Quick's one-stage PT and Owren's method. The latter is most widely used in the Nordic and Benelux countries as well as in Japan, whereas the Quick PT is the approach used elsewhere, accounting for about 95% of all PT tests performed.
  • Pivka protein induced by vitamin K absence or antagonists
  • coumarin therapy is associated with an endogenous competitive coagulation inhibitor, which they later named Pivka.
  • the proteins in question were pre-stages of vitamin K-dependent factors. They inhibited the prothrombin-converting complex, presumably against coagulation factor X (FX) (3).
  • FX coagulation factor X
  • Pivka factors lack gamma carboxyglutamic acid, which is necessary for calcium binding and thereby for “adsorption” of these factors to phospholipid surfaces. Thus, they are inactive analogs to active coagulation factors (4,5).
  • the present invention concerns a method for determining a Pivka corrected prothrombin time (PT) comprising the steps of:
  • the invention also provides a device, such as a coagulation analyzer or Point of Care instrument (POCT), programmed to perform the method of the invention.
  • a device such as a coagulation analyzer or Point of Care instrument (POCT) programmed to perform the method of the invention.
  • POCT Point of Care instrument
  • FIG. 1 The model of Pivka calculation.
  • t min value for normal plasma is constant for one reagent lot.
  • t min value for patient plasma is only for one patient. At least two measurements are needed for one patient sample to calculate the line equation.
  • FIG. 2 Traditional INR (INR Total ) determined by Owren PT, active coagulation factors (INR Corrected ) and inhibition effect (INR Pivka ) for 200 OAT patient plasmas in increasing order using Etaloquick calibration.
  • FIG. 3 PIVKA inhibition (inhibitory factors FII, FVII and FX) on Owren PTs in 200 OAT patient samples as INR units.
  • the present invention provides a method for determining Pivka effect in INR units and a Pivka corrected prothrombin time (PT) comprising the steps of:
  • the INR min or t min value for the samples is obtained by a plot giving the relation between sample dilution or sample volume (X-axis) and clotting time in INR or sec (Y-axis), respectively.
  • a regression line is drawn through the points corresponding to INR's or clotting times of different dilutions or sample volumes of the sample. The regression line intercepts the Y-axis at INR min or t min (see FIG. 1 ).
  • the value for Pivka effect on the measured prothrombin time is calculated by using the equation:
  • INR Pivka INR min (patient sample, calibrator, or control) ⁇ INR min (normal plasma)
  • t Pivka t min (patient sample, calibrator, or control) ⁇ t min (normal plasma).
  • step d) of the method the Pivka effect on the PTs of patient sample is preferably corrected by using one of the following equations:
  • IN corrected INR patient, calibrator, control ⁇ INR Pivka
  • INR patient, calibrator, control or t patient, calibrator, control is a prothrombin time of a sample measured in step a) of the method and wherein INR Pivka or t Pivka is a value calculated in step c) of the method.
  • INR patient, calibrator, control or t patient, calibrator, control is a prothrombin time of an undiluted sample, i.e. INR total or t total , respectively.
  • INR (sample sec /normal sec ) ISI
  • sample sec is a prothrombin time of a patient sample (or a calibrator, or a control sample) measured in seconds
  • normal sec is a prothrombin time of a sample of normal plasma measured in seconds
  • ISI is relative sensitivity of the coagulant reagent used in the PT test. ISI value is usually given by the manufacturer of the reagent or measured using ISI calibrator kits.
  • the plasma samples for the PT test are preferably diluted with a physiologic salt solution or other suitable buffer.
  • sample dilution is not necessary.
  • these mixes of different sample volumes and test reagents are also called herein as “dilutions”.
  • the expression “at least two dilutions” refers herein also to a set of samples wherein one of the samples is an undiluted sample.
  • step b) of the method is performed only once for a certain coagulation reagent (i.e. thromboplastin) and the result obtained is used in step c) for plurality of patient, calibrator, or control samples tested with the same reagent.
  • a certain coagulation reagent i.e. thromboplastin
  • the result obtained is used in step c) for plurality of patient, calibrator, or control samples tested with the same reagent.
  • the inhibitor-free plasma or whole blood sample is taken from a subject known to be healthy (i.e. a sample of normal plasma).
  • the expression “inhibitor-free plasma or whole blood sample” means herein that the plasma or whole blood sample does not contain inhibitors, such as Pivka-inhibitors.
  • the method of the invention can also be performed with a fully automatic coagulation analyser, since current analysers can easily be programmed to run a sample pattern and calculations required for the execution of the present method.
  • the present invention is also directed to a device, such as a coagulation analyser or Point of Care instrument (POCT), programmed to perform the method of the invention.
  • a device such as a coagulation analyser or Point of Care instrument (POCT)
  • POCT Point of Care instrument
  • Devices and methods for assaying coagulation in fluid samples are well-known in the art (see, e.g., U.S. Pat. No. 6,750,053).
  • Point of Care instruments are portable devices developed for rapid determination of prothrombin time (PT) and INR at locations not limited to laboratories, hospitals or health centers. Patients can, e.g., use Point of Care instruments for self-testing at home.
  • the present invention is also directed to a use of a device, such as a coagulation analyzer or Point of Care instrument (POCT), for performing the present method.
  • a device such as a coagulation analyzer or Point of Care instrument (POCT)
  • POCT Point of Care instrument
  • the present invention is further directed to a device or use of said device, such as a computer, for calculating t Pivka or INR Pivka value from the results of the steps a) and b) of the present method, and determining the Pivka corrected PT for the sample of said step a) by subtracting t Pivka or INR Pivka value obtained in step c) of the present method from a prothrombin time measured in said step a).
  • a device or use of said device such as a computer, for calculating t Pivka or INR Pivka value from the results of the steps a) and b) of the present method, and determining the Pivka corrected PT for the sample of said step a) by subtracting t Pivka or INR Pivka value obtained in step c) of the present method from a prothrombin time measured in said step a).
  • the PT coagulation times were measured using a fully automated BCS coagulation analyser (The Dadebehring Coagulation System, Dadebehring, Marburg, Germany).
  • a fully automated BCS coagulation analyser The Dadebehring Coagulation System, Dadebehring, Marburg, Germany.
  • 100 ⁇ L of coagulation reagent was added to 50 ⁇ L of citrated plasma.
  • the four test reagents were:
  • the coagulation reaction contained 10 ⁇ L of citrated sample plasma, 50 ⁇ L of diluent and 150 ⁇ L of reagent.
  • the three test reagents were:
  • Plasma dilutions 1:2 were made with a physiologic salt solution (Natriumklorid 9 mg/mL, 500 ml) from Kabi.
  • the respective CVs were: 2.3% for Neoplastine CL Plus, 2.7% for PT-Fibrinogen Recombinant, 1.1% for PT-Fibrinogen HS Plus, 2.6% for Dade Innovin, 1.4% for Owren's PT, 1.6% for Nycotest PT, and 1.0% for SPA.
  • INR (sample sec /normal sec ) ISI
  • the Microsoft Excel 5.0 program was used to obtain the correlation functions and INR results.
  • the average intercept varies using the Quick PT from 0.03 to 0.14 INR and using the Owren PT 0.01 to 0.03 INR for normal plasmas.
  • the average intercept varies using the Quick PT from 0.40 to 1.46 INR and using the Owren PT 0.20 to 0.28 INR for OAT plasmas.
  • the average SDs of intercepts for normal plasmas (0.07 INR) and OAT plasmas (0.72 INR) using the Quick PT method and the Owren PT were 0.02 INR; 0.23 INR.
  • the average of the Pivka effect on the Quick PT is 0.36 INR (SD 0.43 INR) (without Innovin reagent 0.15 INR; SD 0.14) and on the Owren PT 0.36 INR (SD 0.24 INR).
  • the average INR results from OAT plasmas using Pivka correction were for the Quick PT 2.58 INR (SD 0.11) and for the Owren PT 2.51 (SD 0.16) (Table 1).
  • PT reagents should have low ISI, near 1.0. For this reason we chose sensitive Owren and Quick reagents for this study.
  • the effect of ISI (calibration) as power function grows in the therapeutic range and at higher INR values (9). This makes result harmonisation more demanding in the therapeutic range.
  • the analytical criteria for PT measurement are very tight (bias ⁇ 0.20 INR and CV ⁇ 5%), partly due to the marked biological variation in OAT patients (12).
  • sample needle (Terumo, Venoject needle, Quick Fit, cat. no. MN-2138MQ) was 0.8 ⁇ 40 mm. Sample tubes were centrifuged at 1850 g for 10 min at 20° C. to separate plasma. All measurements were commenced within 8 hours of blood collection.
  • the PT coagulation times were measured using a fully automated BCS coagulation analyser (DadeBehring Coagulation System, DadeBehring, Marburg, Germany).
  • coagulation reagent 100 ⁇ L was added to 50 ⁇ L of citrated plasma and for the dilution sample volumes were 100 ⁇ L+25 ⁇ L+25 ⁇ L (a physiologic salt solution, “Natriumklorid 9 mg/mL”, 500 ml from Kabi).
  • the coagulation reaction contained 10 ⁇ L of citrated sample plasma, 60 ⁇ L of diluent and 140 ⁇ L of reagent and volumes for “dilution measurement”: 5 ⁇ L+65 ⁇ L+140 ⁇ L, 7 ⁇ L+63 ⁇ L+140 ⁇ L or 14 ⁇ L+56 ⁇ L+140 ⁇ L.
  • INR Corrected INR Total ⁇ INR Pivka
  • INR (sample sec /normal sec ) ISI
  • the dilution factors for the Quick PT linearity check were: 0.91; 1.00; 1.25; 1.67 2.00 and the Owren PT linearity check were: 0.67; 1.00; 1.25; 1.67; 2.50.
  • the respective CVs were: 2.6% for Dade Innovin, 1.6% for Nycotest PT. This is consistent with our previous observations with a broader spectrum of reagents (9).
  • the Microsoft Excel 5.0 program was used to obtain the correlation functions and INR results by using the least-squares fit.

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Abstract

The present invention relates to tests for monitoring oral anticoagulation therapy and hepatocellular carcinoma (HCC). Particularly, the invention provides a method for determining prothrombin time of a plasma or whole blood sample taking account the effect which protein induced by vitamin K absence or antagonists (Pivka) has on clotting time and INR result. The primary object of the invention is to harmonise prothrombin time methods for international normalized ratio (INR) results and measure INRpivka.

Description

    FIELD OF THE INVENTION
  • The present invention relates to tests based on INR units for monitoring oral anticoagulation therapy and hepatocellular carcinoma (HCC). Particularly, the invention provides a method for determining prothrombin time of a plasma or whole blood sample taking account the effect which protein induced by vitamin K absence or antagonists (Pivka) has on INR. The object of the invention is to harmonise prothrombin time methods for international normalized ratio (INR) results and also measure Pivka effect as INR units (i.e. INRPivka).
    • BACKGROUND OF THE INVENTION
  • The prothrombin time (PT) test was introduced to control oral anticoagulant therapy (OAT), which is used to treat patients with thrombotic disorders such as thrombophilia. This therapy is based on vitamin K antagonists such as warfarin (or coumarin) inhibiting the synthesis of coagulation factors (F II, F VII, F IX and F X) in the liver. Currently, the need for OAT is increasing worldwide. For example, in Finland warfarin medication was prescribed to 1.7% of the population in 2003 and the number of patients is growing due to the ageing population. Since OAT medication needs continuous control to prevent serious consequences of thrombosis or bleeding, it is not surprising that 800 million PT tests are performed each year throughout the world. The most commonly used PT tests are based on Quick's one-stage PT and Owren's method. The latter is most widely used in the Nordic and Benelux countries as well as in Japan, whereas the Quick PT is the approach used elsewhere, accounting for about 95% of all PT tests performed.
  • When the International Normalised Ratio (INR) and International Sensitivity Index (ISI) were introduced by the World Health Organization (WHO), the aim was to harmonise PT results for oral anticoagulant therapy (5): PT results for a certain plasma or whole blood sample should be the same in INR units regardless of the reagent, instrument or method used. Today each commercial coagulation reagent (i.e. thromboplastin) for PT is calibrated against the primary WHO reference preparation. The results are used to calculate the relative sensitivity of the thromboplastin reagents declared in ISI (International Sensitivity Index). The INR results are then calculated according to the formula: INR=[PT ratio]ISI. However, increasing use of the INR format has led to appreciation of its limitations and recently it was found, that the agreement between a number of (or perhaps most) commercial INR methods is poor and clinically too much INR variation was present, thus compromising the good care of the patients (9,10).
  • Hemker and colleagues (1,2) were the first to characterise the role of protein induced by vitamin K absence or antagonists (Pivka). They discovered that coumarin therapy is associated with an endogenous competitive coagulation inhibitor, which they later named Pivka. The proteins in question were pre-stages of vitamin K-dependent factors. They inhibited the prothrombin-converting complex, presumably against coagulation factor X (FX) (3). It was found that Pivka factors lack gamma carboxyglutamic acid, which is necessary for calcium binding and thereby for “adsorption” of these factors to phospholipid surfaces. Thus, they are inactive analogs to active coagulation factors (4,5).
  • Talstad contemplates the question why the standardisation of PT is a problem and suggests PT standardization by correction of the Pivka inhibitor (15,16). Heckemann et al. discloses a method for simultaneous determination of functional coagulation factors and competitive Pivka-inhibitors based on enzyme kinetics (17). Moreover, immunochemical assays for Pivka are also known (see, e.g., U.S. Pat. No. 5,516,640). However, no simple and practical method for Pivka correction in PT tests has been introduced in the prior art yet. Consequently, the aim of the present invention was to study the Pivka effect further and compare the Quick and the Owren PT methods in view of Pivka by using different reagents. As a result, the present invention provides a straightforward method for PT testing which overcomes the problem of the Pivka effect.
    • SUMMARY OF THE INVENTION
  • The present invention concerns a method for determining a Pivka corrected prothrombin time (PT) comprising the steps of:
      • a) measuring prothrombin time of at least two different dilutions of a plasma or whole blood sample taken from a patient under oral anticoagulant therapy (OAT) or a patient with hepatocellular carcinoma (HCC) or of a calibrator or control plasma sample in order to determine tmin or INRmin value for the sample;
      • b) measuring prothrombin time of at least two different dilutions of a sample of an inhibitor-free plasma or whole blood sample in order to determine tmin or INRmin value for the normal plasma;
      • c) calculating tPivka or INRPivka value from the results of the steps a) and b);
      • d) determining the Pivka corrected PT for the sample of step a) by subtracting tPivka or INRPivka value obtained in step c) from a prothrombin time measured in step a).
  • The invention also provides a device, such as a coagulation analyzer or Point of Care instrument (POCT), programmed to perform the method of the invention.
    • BRIEF DESCRIPTION OF THE DRAWINGS
  • FIG. 1. The model of Pivka calculation. tmin value for normal plasma is constant for one reagent lot. tmin value for patient plasma is only for one patient. At least two measurements are needed for one patient sample to calculate the line equation.
  • FIG. 2. Traditional INR (INRTotal) determined by Owren PT, active coagulation factors (INRCorrected) and inhibition effect (INRPivka) for 200 OAT patient plasmas in increasing order using Etaloquick calibration.
  • FIG. 3. PIVKA inhibition (inhibitory factors FII, FVII and FX) on Owren PTs in 200 OAT patient samples as INR units.
    •  DETAILED DESCRIPTION OF THE INVENTION
  • The present invention provides a method for determining Pivka effect in INR units and a Pivka corrected prothrombin time (PT) comprising the steps of:
      • a) measuring prothrombin time of at least two different dilutions of a plasma or whole blood sample taken from a patient under oral anticoagulant therapy (OAT) or a patient with hepatocellular carcinoma (HCC) or of a calibrator or control plasma sample in order to determine tmin or INRmin value for the sample;
      • b) measuring prothrombin time of at least two different dilutions of an inhibitor-free plasma or whole blood sample in order to determine tmin or INRmin value for the normal plasma;
      • c) calculating tPivka or INRPivka value from the results of the steps a) and b);
      • d) determining the Pivka corrected PT for the sample of step a) by subtracting tPivka or INRPivka value obtained in step c) from a prothrombin time measured in step a).
  • The INRmin or tmin value for the samples is obtained by a plot giving the relation between sample dilution or sample volume (X-axis) and clotting time in INR or sec (Y-axis), respectively. A regression line is drawn through the points corresponding to INR's or clotting times of different dilutions or sample volumes of the sample. The regression line intercepts the Y-axis at INRmin or tmin (see FIG. 1).
  • Preferably, the value for Pivka effect on the measured prothrombin time is calculated by using the equation:

  • INR Pivka =INR min (patient sample, calibrator, or control)−INR min(normal plasma)
  • or

  • t Pivka =t min(patient sample, calibrator, or control)−t min(normal plasma).
  • It is also possible to convert the tPivka value to the INR units.
  • In step d) of the method the Pivka effect on the PTs of patient sample is preferably corrected by using one of the following equations:

  • IN corrected =INR patient, calibrator, control −INR Pivka
  • or

  • t corrected =t patient, calibrator, control −t pivka
  • wherein INRpatient, calibrator, control or tpatient, calibrator, control is a prothrombin time of a sample measured in step a) of the method and wherein INRPivka or tPivka is a value calculated in step c) of the method. Preferably said INRpatient, calibrator, control or tpatient, calibrator, control is a prothrombin time of an undiluted sample, i.e. INRtotal or ttotal, respectively.
  • Initial INR values for the PT samples are calculated with the formula of:

  • INR=(samplesec/normalsec)ISI
  • wherein samplesec is a prothrombin time of a patient sample (or a calibrator, or a control sample) measured in seconds, normalsec is a prothrombin time of a sample of normal plasma measured in seconds, and ISI is relative sensitivity of the coagulant reagent used in the PT test. ISI value is usually given by the manufacturer of the reagent or measured using ISI calibrator kits.
  • The plasma samples for the PT test are preferably diluted with a physiologic salt solution or other suitable buffer. However, when using different sample volumes for the measurement, the sample dilution is not necessary. For the sake of simplicity, these mixes of different sample volumes and test reagents are also called herein as “dilutions”. Furthermore, the expression “at least two dilutions” refers herein also to a set of samples wherein one of the samples is an undiluted sample.
  • Preferably, step b) of the method is performed only once for a certain coagulation reagent (i.e. thromboplastin) and the result obtained is used in step c) for plurality of patient, calibrator, or control samples tested with the same reagent. This is possible since normal plasma does not contain Pivka and, thus, the tmin or INRmin value of normal plasma is always a constant for a certain coagulation reagent. Preferably, in step b) the inhibitor-free plasma or whole blood sample is taken from a subject known to be healthy (i.e. a sample of normal plasma). The expression “inhibitor-free plasma or whole blood sample” means herein that the plasma or whole blood sample does not contain inhibitors, such as Pivka-inhibitors.
  • The method of the invention can also be performed with a fully automatic coagulation analyser, since current analysers can easily be programmed to run a sample pattern and calculations required for the execution of the present method. Thus, the present invention is also directed to a device, such as a coagulation analyser or Point of Care instrument (POCT), programmed to perform the method of the invention. Devices and methods for assaying coagulation in fluid samples are well-known in the art (see, e.g., U.S. Pat. No. 6,750,053). Point of Care instruments are portable devices developed for rapid determination of prothrombin time (PT) and INR at locations not limited to laboratories, hospitals or health centers. Patients can, e.g., use Point of Care instruments for self-testing at home.
  • The present invention is also directed to a use of a device, such as a coagulation analyzer or Point of Care instrument (POCT), for performing the present method.
  • The present invention is further directed to a device or use of said device, such as a computer, for calculating tPivka or INRPivka value from the results of the steps a) and b) of the present method, and determining the Pivka corrected PT for the sample of said step a) by subtracting tPivka or INRPivka value obtained in step c) of the present method from a prothrombin time measured in said step a).
    • EXPERIMENTAL SECTION EXAMPLE 1 Materials and Methods Patients and Blood Sampling
  • All procedures were approved by our institution's responsible committee in accordance with the Helsinki Declaration of 1975. We analysed normal and OAT patient samples chosen without conscious bias from among hospital and health center patients. Blood (1.8 mL) was drawn from 10 normal and 10 OAT patients into citrate coagulation tubes (Greiner Labortechnik GmbH, Vacuette cat. no. 454322, 9NC) containing 0.2 mL 0.109 mol/L (3.2%) citrate solution. The sample needle (Terumo, Venoject needle, Quick Fit, cat. no. MN-2138MQ) was 0.8×40 mm. Sample tubes were centrifuged at 1850 g for 10 min at 20° C. to separate plasma. All measurements commenced within 8 hours of blood collection at same time.
    • PT Time Determination
  • The PT coagulation times were measured using a fully automated BCS coagulation analyser (The Dadebehring Coagulation System, Dadebehring, Marburg, Germany). For the one-stage propthrombin time with Quick, 100 μL of coagulation reagent was added to 50 μL of citrated plasma. The four test reagents were:
      • (i) Neoplastine CL Plus, cat. no. 00376 (rabbit brain thromboplastin, Diagnostica Stago), lot 031581, ISI 1.30 (no instrument mentioned), ISI values 1.42;
      • (ii) PT-Fibrinogen Recombinant, cat. no. 20005000 (recombinant rabbit tissue thromboplastin, Instrumentation Laboratory, IL), lot NO 425869, ISI 1.03 for ACL, ISI value 1.08;
      • (iii) PT-Fibrinogen HS Plus, cat. no. 08469810 (rabbit brain thromboplastin, Instrumentation Laboratory, IL), lot NO325729, ISI 1.13 for ACL, ISI value 1.25;
      • (iv) Dade Innovin cat. no. B4212-50 (recombinant human tissue thromboplastin, DadeBehring Marburg GmbH), lot 526987, ISI for BCS 0.90, ISI value 1.04.
  • For the Owren PT (combined thromboplastin reagent) the coagulation reaction contained 10 μL of citrated sample plasma, 50 μL of diluent and 150 μL of reagent. The three test reagents were:
      • (v) Owren's PT, cat. no. GHI (Global Hemostasis Institute) 131-10 (rabbit brain thromboplastin) containing 25 mmol/L of CaCl2 (cat. no. GHI 155) and a diluent (Owren's buffer, cat. no. GHI 150) from the GHI, lot C414F, ISI 1.09 for optical methods, ISI value 1.17;
      • (vi) Nycotest PT, cat. no. 1002488 (rabbit brain thromboplastin) and a diluent (Nycotest PT, dilution liquid, cat. no. 1002485) from Axis-Shield as, lot 10107353, ISI 1.13 for Thrombotrack, ISI value 0.95;
      • (vii) SPA, 50 cat. no. 00105 (tissue thromboplastin) and a diluent (SPA buffer cat. no. 00124) from Diagnostica Stago, lot 022071, ISI 0.98 (no instrument mentioned), ISI value 0.93.
  • The two methods (4+3 reagents) were calibrated for ISI with the same calibrators Etaloquick cat. no. 00496 from Diagnostica Stago lot 021964.
  • Plasma dilutions 1:2 were made with a physiologic salt solution (Natriumklorid 9 mg/mL, 500 ml) from Kabi.
    • Analytical Imprecision of PT Determinations
  • The within-run imprecision of seven PT tests was measured using one patient plasma sample (n=10 determinations) with an INR value in the therapeutic range, i.e., about 2.2 INR. The respective CVs were: 2.3% for Neoplastine CL Plus, 2.7% for PT-Fibrinogen Recombinant, 1.1% for PT-Fibrinogen HS Plus, 2.6% for Dade Innovin, 1.4% for Owren's PT, 1.6% for Nycotest PT, and 1.0% for SPA.
    • Pivka Determination and Statistics
  • We plotted the clotting time (s) on the y-axis and plasma dilution on the x-axis for normal and OAT plasmas. From line equation we got the line intercept at the y-axis, which is the so-called minimal clotting time (tmin) with an infinite number of clotting factors for one sample (3.11). The difference in intercepts (y-axis) between normal plasma and OAT plasma indicates the action of Pivka in seconds without calibration effect. We calculated the difference in intercepts as INR units (OAT intercept—normal plasma intercept, FIG. 1).
  • INR results were calculated in seconds using the formula:

  • INR=(samplesec/normalsec)ISI
  • The Microsoft Excel 5.0 program was used to obtain the correlation functions and INR results.
    • Results
  • The average intercept varies using the Quick PT from 0.03 to 0.14 INR and using the Owren PT 0.01 to 0.03 INR for normal plasmas. The average intercept varies using the Quick PT from 0.40 to 1.46 INR and using the Owren PT 0.20 to 0.28 INR for OAT plasmas. The average SDs of intercepts for normal plasmas (0.07 INR) and OAT plasmas (0.72 INR) using the Quick PT method and the Owren PT were 0.02 INR; 0.23 INR. The average of the Pivka effect on the Quick PT is 0.36 INR (SD 0.43 INR) (without Innovin reagent 0.15 INR; SD 0.14) and on the Owren PT 0.36 INR (SD 0.24 INR). The average INR results from OAT plasmas using Pivka correction were for the Quick PT 2.58 INR (SD 0.11) and for the Owren PT 2.51 (SD 0.16) (Table 1).
    • Discussion
  • Harmonisation of INR results is an essential aim in improving patient care and the usefulness of the scientific literature. The therapeutic ranges in INR units for patient care are harmonised and easy for doctors to use. The problem is to unify INR results all over the world, and this is a task for clinical laboratories. In practise laboratories use manufacturer's ISI for an instrument, manufacturer's or “local” (certain country or area) calibrator kits. INR results from same sample should none the less be the same. The ISI calibration is in key position in harmonising INR results. The variability of PT reagents (thromboplastin, pH, ionic concentrations and quality, additives etc.) globally is considerable and this makes INR harmonisation very difficult.
  • PT reagents should have low ISI, near 1.0. For this reason we chose sensitive Owren and Quick reagents for this study. The effect of ISI (calibration) as power function grows in the therapeutic range and at higher INR values (9). This makes result harmonisation more demanding in the therapeutic range. The analytical criteria for PT measurement are very tight (bias≦0.20 INR and CV<5%), partly due to the marked biological variation in OAT patients (12).
  • Pivka factors have a marked role in the harmonisation of INR results by reason of the effect on calibration in the therapeutic area and the measurement itself. We may observe the Pivka and PT method relationship if we exclude Innovin results (human thromboplastin): the average of Pivka for the Quick PT is 0.15 INR and for the Owren PT 0.36 INR. This means more PIVKA sensitivity and more inhibition (0.21 INR) for the Owren PT method (Table 1). This explains the lower INR results for the Owren compared to the Quick PT (6,13,14). In anticoagulant therapy patients receive more medication (0.21 INR) using Owren PT for care control.
  • In both methods the same manufacturer, Diagnostica Stago, has reagents with very low Pivka sensitivity. We found the greatest Pivka effect using Innovin (0.98 INR), which reagent contains recombinant human tissue thromboplastin while all other reagents contain thromboplastin of rabbit origin. The Pivka varies using different reagents and is partly thromboplastin-dependent. Intercept SDs for normal and OAT plasmas vary clearly more for the Quick PT (0.03 to 0.14 INR, 0.40 to 1.46 INR) than for the Owren PT (0.01 to 0.03 INR, 0.20 to 0.28 INR) (Table 1). These results confirm our view that using the Owren PT method we can harmonise INR results better globally for different reagents. According to our earlier findings we concluded that Owren PT methods are superior (6,7,8).
  • In Table 1 we see almost the same results and minimal dispersion between averages of INR results from OAT plasmas minus Pivka inhibition using different PT reagents and methods. This confirms that the Pivka calculations are correct (the same calibration for all reagents). Pivka inhibition causes problems in INR result harmonization globally (calibration, different reagents, instruments and PT methods)(9). ISI calibrators (the higher INR values) from OAT patients contain also Pivka coagulation factors, which complicates INR system. INR values of calibrators should be without Pivka effect.
  • The method of the present invention needs only at least two PT measurements for one patient sample of different dilutions and simple mathematical calculations. Consequently, the method is easy to adapt to a different kind of instruments. Theoretically PT methods should measure the total effect of anticoagulant drugs on blood coagulation, including active K-dependent clotting factors and inactive factors (Pivka inhibition). This methodological choice means use of Pivka sensitive thromboplastin and method to measure the sum of active and inactive coagulation factors. The another methodological possibility is measure only the active coagulation factors without coagulation inhibitors as in this study. This new method helps to develop the INR system for the best principal possibility to harmonize INRs for oral anticoagulant treatment globally.
    • EXAMPLE 2 Materials and Methods Patients and Blood Sampling
  • Venous blood samples were obtained from 10 normal subjects and 210 hospital and health-centre patients for whom the PT time test was requested for the monitoring of oral anticoagulant therapy. In our region a “P-INR” test code is used for this purpose. Hence, the patient samples represented all possible phases of anticoagulation: (i) before treatment, (ii) dose-adjusting phase, and (iii) the steady-state phase. All procedures were approved by our institution's responsible committee in accordance with the Helsinki Declaration of 1975. Blood (1.8 mL) was drawn into citrate coagulation tubes (Greiner Labortechnik GmbH, Vacuette cat. no. 454322, 9NC) containing 0.2 mL 0.109 mol/L (3.2%) citrate solution. The sample needle (Terumo, Venoject needle, Quick Fit, cat. no. MN-2138MQ) was 0.8×40 mm. Sample tubes were centrifuged at 1850 g for 10 min at 20° C. to separate plasma. All measurements were commenced within 8 hours of blood collection.
    • PT Determination
  • The PT coagulation times were measured using a fully automated BCS coagulation analyser (DadeBehring Coagulation System, DadeBehring, Marburg, Germany).
  • For the one-stage prothrombin time with Quick, 100 μL of coagulation reagent was added to 50 μL of citrated plasma and for the dilution sample volumes were 100 μL+25 μL+25 μL (a physiologic salt solution, “Natriumklorid 9 mg/mL”, 500 ml from Kabi). The test reagent was: Dade Innovin cat. no. B4212-50 (recombinant human tissue thromboplastin, DadeBehring Marburg GmbH), lot 536928, ISI=0.92.
  • For the Owren PT (combined thromboplastin reagent) the coagulation reaction contained 10 μL of citrated sample plasma, 60 μL of diluent and 140 μL of reagent and volumes for “dilution measurement”: 5 μL+65 μL+140 μL, 7 μL+63 μL+140 μL or 14 μL+56 μL+140 μL. The test reagent was: Nycotest PT, cat. no. 1002488 (rabbit brain thromboplastin) and a diluent (Nycotest PT, dilution liquid, cat. no. 1002485) from Axis-Shield as, lot 10112954, ISI=1.07.
    • ISI Calibration
  • Two local ISI calibrator kits were used: (i) “Svensk nationell kalibrator för protrombinkomplexaktiviet”, from Equalis, lot 11, 12, Cal 1=0.85 INR and Cal 2=3.19 INR (used mainly in Sweden and Norway). (ii) “ISI-kalibraattorikitti”, cat. no. B10000150, from Bioclin, lot 8, Cal 1=2.07 INR, Cal 2=3.52 INR and Cal 3=1.0 INR (used mainly in Finland).
  • Further, two commercial (manufacturer calibration) ISI calibration kits were used: (i) Etaloquick cat. no. 00496 from Diagnostica Stago lot 041555. Cal 1=0.91 INR, Cal 2=3.24 INR and Cal 3=4.90 INR. (ii) PT-Multi Calibrator cat. no. OPAT 035 from DadeBehring lot 35422. Cal 1=1.01 INR, Cal 2=1.30 INR, Cal 3=1.65 INR, Cal 4=2.97 INR, Cal 5=4.00 INR, Cal 6=5.29 INR.
    • Determination of Minimal PT Time and Respective INR
  • The procedure for measuring the inhibition in seconds was conducted essentially as described by Hemker and co-workers (1,2,3). We constructed PT (sec) versus D (D=plasma or calibrator dilution factor) plots for normal and OAT plasmas as well as for different calibrators. This is consistent with an uncompetitive inhibition principle with oral anticoagulants (18). From the line equation the y-axis intercept is calculated. This is the so-called minimal clotting time (tmin) with an infinite number of clotting factors (3). The difference in intercepts (y-axis) between normal plasma and OAT plasma indicates the action of PIVKA in seconds without calibration effect. We furthermore calculated the difference in intercepts also in INR units and subtracted it from total INR:

  • INR Corrected =INR Total −INR Pivka
  • INR's were calculated using the formula: INR=(samplesec/normalsec)ISI
  • The dilution factors for the Quick PT linearity check were: 0.91; 1.00; 1.25; 1.67 2.00 and the Owren PT linearity check were: 0.67; 1.00; 1.25; 1.67; 2.50.
    • Analytical Imprecision and Statistics
  • The within-run precision of PT tests was measured using one patient plasma sample (n=10 determinations) with an INR value in the therapeutic range, i.e., approx. 2.2 INR. The respective CVs were: 2.6% for Dade Innovin, 1.6% for Nycotest PT. This is consistent with our previous observations with a broader spectrum of reagents (9). The Microsoft Excel 5.0 program was used to obtain the correlation functions and INR results by using the least-squares fit.
    • Results
  • PIVKA inhibition was demonstrable in all calibrators with INR values greater than 1. As expected, the inhibition increased together with the increase in calibrator INR value (Table 2). It is noteworthy, however, that the PIVKA inhibition varied among the calibrator kits and was different for the two different PT methods.
  • We further demonstrated that there was a conspicuous difference in INR results in the case of 200 OAT patients, depending on the PT method, even if the same calibrator was used. The average for traditional INR was 3.89 and 2.68 when determined by the Quick and Owren method, respectively. After PIVKA correction the averages were 2.49 and 2.30 INR units, representing INRCorrected. These results allowed us to estimate the target point of 2.13 INRCorrected units, the range being 1.6-2.6 INRCorrected units.
  • The linearity using different dilutions was good for the Quick and Owren PT methods. We further demonstrated that there was a difference—increasing towards higher INR values—between the traditional PT measurement and the new method measuring the active coagulation (INRCorrected) in the case of the 200 OAT patients. Individual original and corrected (INRCorrected) values are illustrated in FIG. 2. The individual variation in coagulation inhibition is notable at different INR levels (Owren PT) for OAT patient samples as illustrated in FIG. 3.
    • Discussion
  • This new method requires two PT measurements for one patient sample and mathematical calculations: INRpatient, calibrator, or control−INRPivka=INRCorrected. It is easy to adapt for different kinds of instruments. The reagent costs are the same using a half volume for PT measurements, as automation instruments can pipet very low liquid volumes.
  • TABLE 1
    Measuring Pivka inhibition using the Quick and Owren PT methods and different reagents for both methods.
    Average equation Intercept SD Average equation Intercept SD Average Average of
    Etaloquick of normal plasma of normal of OAT plasma of OAT Pivka of OAT OAT plasma
    calibration (s), n = 10 plasma (INR) (s), n = 10 plasma (INR) (INR) plasma minus Pivka
    The Quick PT
    Innovin y = 2.92x + 5.63 0.05 y = 15.05x + 14.53 0.59 0.98 3.41 2.43
    PT Fibrinogen y = 8.37x + 7.53 0.14 y = 32.59x + 10.46 1.46 0.19 2.88 2.69
    Recomb
    PT Fibrinogen y = 7.45x + 8.48 0.03 y = 25.98x + 12.56 0.41 0.27 2.87 2.60
    HS Plus
    Neoplastin y = 9x + 4.42 0.07 y = 27.66x + 3.84 0.40 −0.02 2.62 2.64
    Average 0.07 0.72 0.36 2.95 2.59
    SD 0.43 0.33 0.11
    The Owren PT
    SPA Y = 9.15x + 13.37 0.03 y = 52.58x + 15.58 0.21 0.09 2.78 2.69
    Nycotest PT y = 8.7x + 11.98 0.02 y = 44.63x + 21.84 0.20 0.44 2.93 2.49
    Owren PT Y = 8.76x + 15.98 0.01 y = 35.8x + 28.69 0.28 0.56 2.92 2.36
    Average 0.02 0.23 0.36 2.88 2.51
    SD 0.24 0.09 0.16
  • TABLE 2
    INR inhibition obtained with four calibrator kits using two different PT methods
    Quick PT Owren PT
    Calibratora Calibrator INRb INR inhibitionc INRd cor Inhibition (%) INR inhibitionc INRd cor Inhibition (%)
    Multical 1 1.01 0.00 1.01 None 0.00 1.01 None
    Multical
    2 1.30 0.13 1.17 10.07 0.04 1.26 3.29
    Multical 3 1.66 0.27 1.39 16.09 0.11 1.55 6.76
    Multical 4 2.93 0.70 2.23 23.86 0.29 2.64 9.74
    Multical 5 4.14 1.14 3.00 27.53 0.49 3.65 11.90
    Multical 6 5.46 1.85 3.61 33.91 1.12 4.34 20.43
    Etaloquick 1 1.00 0.00 1.00 None 0.00 1.00 None
    Etaloquick
    2 2.85 0.63 2.22 22.13 0.31 2.54 10.78
    Etaloquick 3 4.25 1.16 3.09 27.24 1.00 3.25 23.59
    Bioclin 3 1.00 0.00 1.00 None 0.00 1.00 None
    Bioclin
    1 2.07 0.12 1.95 5.78 0.32 1.75 15.36
    Bioclin 2 3.52 0.80 2.72 22.86 0.74 2.78 21.10
    Equalis 1 0.85 0.00 0.85 None 0.00 0.85 None
    Equalis
    2 3.19 0.28 2.91 8.78 0.31 2.88 9.69
    aArranged according to increasing INR values.
    bAs given by the manufacturer.
    cWe constructed INR (y-axis) versus C (C = calibrator dilution factor) (x-axis) plots for each calibrator. The inhibition was calculated by subtracting, in turn, the y-axis intercept (INR) value of each respective calibrator of the lowest INR value from calibrators with higher values, i.e., containing PIVKA. For details, see Materials and Methods and FIG. 1.
    dRepresents the y-axis intercept of the INR versus 1/C line, i.e., the hypothetical clotting time or INRCorrected with no inhibitors present.
    • REFERENCES
    • 1. Hemker H C, Veltkamp J J, Hensen A, Loeliger E A. Nature of Prothrombin Biosynthesis: Preprothrombinemia in Vitamin K-deficiency. Nature 1963; 200:590-8.
    • 2. Hemker HC. Preprothrombin (complex?) a circulating anticoagulant in coumarin treated and vitamin K deficient patients. Thrombos Diathes Haemorrh Suppl 1964; 13:380.
    • 3. Henker H C, Muller A D. Kinetic Aspects of the Interaction of Blood-Clotting Enzymes. VI. Localization of the Site of Blood-Coagulation Inhibition by the Protein Induced by Vitamin K Absence (PIVKA). Thrombos Diathes Haemorrh 1968; 20:78-87.
    • 4. Stenflo J. Vitamin K, prothrombin and g-carboxyglutamatic acid. New Eng J Med 1977; 296:624.
    • 5. Hirsh J, Dalen J E, Anderson D R, Poller L, Bussey H, Ansell J et al. Oral Anticoagulants Mechanism of Action, Clinical Effectiveness, and Optimal Therapeutic Range. Chest 1998; 114:445-69.
    • 6. Horsti J. Agreement of Owren and Quick Prothrombin Times: Effects of Citrate and Calcium Concentrations and International Sensitivity Index Correction. Clin Chem 2001; 47:940-4.
    • 7. Horsti J. Comparison of Quick and Owren Prothrombin Time with Regard to the Harmonisation of the International Normalised Ration (INR) System. Clin Chem Lab Med 2002; 40:399-403.
    • 8. Horsti J. Has Quick or Owren prothrombin time method the advantage in harmonisation for the International Normalized Ratio system? Blood Coag Fibriol 2002; 13:641-6.
    • 9. Horsti J, Uppa H, Vilpo J. Poor agreement between different prothrombin time International Normalized Ratio (INR) methods: comparison of seven commercial reagents. Clin Chem 2005; 51:553-60.
    • 10. Jackson C M, Esnouf M P. Has the Time Arrived to Replace the Quick Prothrombin Time Test for Monitoring Oral Anticoagulant Therapy. Clin Chem 2005; 51:483-5.
    • 11. Hemker H C, Veltkamp J J, Loeliger E A. Kinetic aspects of the interaction of blood clotting enzymes.3. Demonstration of an inhibitor of prothrombin conversion in vitamin K deficiency. Thromb Diath Haemorrh. 1968; 19:346-63.
    • 12. Kjeldsen J, Lassen J F, Petersen P H, Brandslund I. Biological variation of International Normalised Ratio for prothrombin times, and consequences in monitoring oral anticoagulant therapy: computer simulation of serial measurements with goal-setting for analytical quality. Clin Chem 1997; 43:2175-82.
    • 13. Horsti J. The Quick and Owren prothrombin time methods for oral anticoagulant therapy do not agree well using the International Normalized Ratio (INR) units. Scand J Clin Lab Invest 2003; 63:455-6.
    • 14. Odén A, Fahlén M. Oral anticoagulation and risk of death: a medical record linkage study. BMJ 2002; 325:1073-5.
    • 15. Talstad I. Prothrombin time standardization by correction of the Pivka inhibitor. Haemostasis 1996; 25(5):266-275.
    • 16. Talstad I. Why is the standardization of prothrombin time a problem? Haemostasis 2000; 30(5):258-267.
    • 17. Heckemann H. -J., Ruby Ch. and Rossner K. Simultaneous Determination of Functional Coagulation Factors and Competitive (PIVKA-) Inhibitors Based on Enzyme Kinetics. Folia Haematol., Leipzig 1988; 115(4):533-537.
    • 18. Henry J B. Clinical Diagnosis and Management by Laboratory Methods. 20th ed. Philadelphia: W.B. Saunders Company, 2001:284-5.

Claims (8)

1. Method for determining a Pivka-corrected prothrombin time (PT) comprising the steps of:
a) measuring prothrombin time of at least two different dilutions of a plasma or whole blood sample taken from a patient under oral anticoagulant therapy (OAT) or a patient with hepatocellular carcinoma (HCC) or of a calibrator or control plasma sample in order to determine tmin or INRmin value for the sample;
b) measuring prothrombin time of at least two different dilutions of an inhibitor-free plasma or whole blood sample in order to determine tmin or INRmin value for the normal plasma;
c) calculating tPivka or INRPivka value from the results of the steps a) and b);
d) determining the Pivka corrected PT for the sample of step a) by subtracting tPivka or INRPivka value obtained in step c) from a prothrombin time measured in step a).
2. The method according to claim 1, wherein the Pivka corrected PT for the sample of step a) is determined in step d) by using one of the following equations:

INR corrected =INR patient, calibrator, control −INR Pivka
or

t corrected =t patient, calibrator, control −t Pivka
wherein INRpatient, calibrator, control or tpatient, calibrator, control is a PT of a sample measured in step a) of the method, and wherein INRPivka or tPivka is a value calculated in step c) of the method.
3. The method according to claim 1, wherein it is performed with a fully automatic coagulation analyser programmed to run a sample pattern and calculations required for the execution of the method.
4. The method according to claim 1, wherein step b) is performed once for a certain coagulation reagent (i.e. thromboplastin) and the result obtained is used in step c) for plurality of patient, calibration or control samples tested with the same reagent.
5. Use of a device for performing the method according to claim 1.
6. The use according to claim 5, wherein said device is a coagulation analyzer or Point of Care instrument (POCT).
7. Use of a device for calculating tPivka or INRPivka value from the results of the steps a) and b) of the method according to claim 1, and determining the Pivka corrected PT for the sample of said step a) by subtracting tPivka or INRPivka value obtained in step c) of the method according to claim 1 from a prothrombin time measured in said step a).
8. The use according to claim 7, wherein said device is a computer.
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